Difference between revisions of "Template:UPMC-Paris/Test"

Latest revision as of 15:07, 29 July 2016

MENU ▤

Competent Cells
- Preparation of Bacillus subtilis competent cells
  1. Streak out the strain to be made competent on an LB agar plate as a large patch and incubate overnight at 30°C
  2. The following morning scrape the cell growth off the plate and use to inoculate fresh, pre-warmed, SpC medium (20 ml) to give an OD600 reading of about 0.5.
  3. Incubate the culture at 37°C with vigorous aeration and take periodic OD readings (OD600) to assess cell growth.
  4. When the rate of cell growth is seen to depart from exponential (i.e. no significant change in cell density over 20-30 min) inoculate 200 ml of pre-warmed, SpII medium with 2 ml of stationary-phase culture and continue incubation at 37°C with slower aeration
  5. After 90 min incubation, pellet the cells by centrifugation (8,000 g, 5min) at room temperature.
  6. Carefully decant the supernatant into a sterile container and save.
  7. Gently resuspended the cell pellet in 18 ml of the saved supernatant and add 2 ml of sterile glycerol; mix gently
  8. Aliquot the competent cell (0.5 ml) in sterile tubes, freeze rapidly in liquid nitrogen or a dry-iced/ethanol bath or ice/isopropanol bath and store -70.
Transformation
- Cells Preparation :
  1. Thaw competent cells rapidly by immersing frozen tubes in a 37°C water bath
  2. Immediately, add one volume of SpII + EGTA to the Thawed cells; mix gently
  3. In a sterile test tube add competent cell (0.2~0.5 ml) to the DNA solution (<0.1 ml) and incubate in a roller drum at 37.
  4. Dilute the transformed cells as appropriate in T base containing 0.5% glucose and plate immediately onto selective media.
  Digestion :
  1. Select restriction enzymes to digest your plasmid. Determine an appropriate reaction buffer by reading the instructions for your enzyme.
  2. Incubate tube at appropriate temperature (usually 37°C) for 1 hour.
  3. Always follow the manufacturer’s instructions.
  4. To visualize the results of your digest, conduct gel electrophoresis
  Vector Preparation :
  Combine the following in a PCR or Eppendorf tube:
  - 25ng Vector DNA
  - 75ng Insert DNA
  - Ligase Buffer (1μL/10μL reaction for 10X buffer, and 2μL/10μL reaction for 5X buffer)
  - 0.5-1μL T4 DNA Ligase
  - H20 to a total of 10μL
  Incubate at room temperature for 2hr, or at 16°C overnight (following the manufacturer’s instructions).
Deletion
- Deletion Step 1 :
  
  Deletion Step 2 :
  
  Deletion Step 3 :
Other
- Whatever Step 1 :
  
  Whatever Step 2 :
  
  Un autre truc Step 1 :
  
  Un autre truc Step 2 :

@@ Line 382: / Line 382: @@
-<li class="menu_item"> <div class="icon plus"></div> Competent Cells :
+<li class="menu_item"> <div class="icon plus"></div> Competent Cells
 <ul class="submenu">
 <li>
 <a href="">
 <div>
-<p>Competency Step 1 :</p>
+<h>Preparation of Bacillus subtilis competent cells</h>
-<img src="aaa" width="500px"/>
-<p>Competency Step 2 :</p>
-<img src="aaa" width="500px"/>
-<p>Competency Step 3 :</p>
-<img src="aaa" width="500px"/></div></a></li></ul></li>
+<ol><li>Streak out the strain to be made competent on an LB agar plate as a large patch and incubate overnight at 30°C</li>
-<li class="menu_item"> <div class="icon plus"></div> Transformation :
+<li>The following morning scrape the cell growth off the plate and use to inoculate fresh, pre-warmed, SpC medium (20 ml) to give an OD600 reading of about 0.5. </li>
+<li>Incubate the culture at 37°C with vigorous aeration and take periodic OD readings (OD600) to assess cell growth.</li>
+<li>When the rate of cell growth is seen to depart from exponential (i.e. no significant change in cell density over 20-30 min) inoculate 200 ml of pre-warmed, SpII medium with 2 ml of stationary-phase culture and continue incubation at 37°C with slower aeration </li>
+<li>After 90 min incubation, pellet the cells by centrifugation (8,000 g, 5min) at room temperature.</li>
+<li>Carefully decant the supernatant into a sterile container and save.</li>
+<li>Gently resuspended the cell pellet in 18 ml of the saved supernatant and add 2 ml of sterile glycerol; mix gently </li>
+<li>Aliquot the competent cell (0.5 ml) in sterile tubes, freeze rapidly in liquid nitrogen or a dry-iced/ethanol bath or ice/isopropanol bath and store -70.</li></ol>
+</div></a></li></ul></li>
+<li class="menu_item"> <div class="icon plus"></div> Transformation
 <ul class="submenu">
 <li>
 <a href="">
 <div>
-<p>Transformation Step 1 :</p>
+<h>Cells Preparation :</h>
-<img src="aaa" width="500px"/>
-<p>Transformation Step 2 :</p>
-<img src="aaa" width="500px"/>
-<p>Transformation Step 3 :</p>
-<img src="aaa" width="500px"/></div></a></li></ul></li>
+<ol><li>Thaw competent cells rapidly by immersing frozen tubes in a 37°C water bath</li>
+<li>Immediately, add one volume of SpII + EGTA to the Thawed cells; mix gently </li>
-<li class="menu_item"> <div class="icon plus"></div> Deletion :
+<li>In a sterile test tube add competent cell (0.2~0.5 ml) to the DNA solution (<0.1 ml) and incubate in a roller drum at 37.</li>
+<li>Dilute the transformed cells as appropriate in T base containing 0.5% glucose and plate immediately onto selective media. </li></ol>
+<p align="center"><img src="https://static.igem.org/mediawiki/igem.org/d/d3/Transfo_pic_1.png" width="400px"/></p>
+</div></a>
+<a href=""><div>
+<h>Digestion :</h>
+<ol><li>Select restriction enzymes to digest your plasmid. Determine an appropriate reaction buffer by reading the instructions for your enzyme. </li>
+<p>In a 1.5mL tube combine the following:</p>
+<ul><li>DNA </li>
+<li>Restriction Enzyme(s)</li>
+<li>Buffer </li>
+<li>dH2O up to total volume</li> </ul>
+<p>Mix gently by pipetting. </p>
+<li>Incubate tube at appropriate temperature (usually 37°C) for 1 hour. </li>
+<li>Always follow the manufacturer’s instructions. </li>
+<li>To visualize the results of your digest, conduct gel electrophoresis</li></ol>
+</div></a>
+<a href=""><div>
+<h>Vector Preparation :</h>
+<p>Combine the following in a PCR or Eppendorf tube:</p>
+<ul><li>25ng Vector DNA</li>
+<li>75ng Insert DNA</li>
+<li>Ligase Buffer (1μL/10μL reaction for 10X buffer, and 2μL/10μL reaction for 5X buffer)</li>
+<li>0.5-1μL T4 DNA Ligase</li>
+<li>H20 to a total of 10μL</li></ul>
+<p>Incubate at room temperature for 2hr, or at 16°C overnight (following the manufacturer’s instructions).</p>
+</div></a></li></ul></li>
+<li class="menu_item"> <div class="icon plus"></div> Deletion
 <ul class="submenu">
 <li>
@@ Line 422: / Line 468: @@
-<li class="menu_item"> <div class="icon plus"></div> Other :
+<li class="menu_item"> <div class="icon plus"></div> Other
 <ul class="submenu">
 <li>
@@ Line 428: / Line 474: @@
 <div>
 <p>Whatever Step 1 :</p>
-<img src="aaa" width="500px"/>
+<img src="aaa" width="50px"/>
 <p>Whatever Step 2 :</p>
-<img src="aaa" width="500px"/></div>
+<img src="aaa" width="50px"/></div></a>
+<a href="">
 <div>
 <p>Un autre truc Step 1 :</p>
-<img src="aaa" width="500px"/>
+<img src="aaa" width="50px"/>
 <p>Un autre truc Step 2 :</p>
-<img src="aaa" width="500px"/></div></a></li></ul></li>
+<img src="aaa" width="50px"/></div></a></li></ul></li>